Last updated: 2019-09-04
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Knit directory: apaQTL/analysis/
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Unstaged changes:
Modified: analysis/NuclearSpecAPAqtl.Rmd
Modified: analysis/PrematureTermQTL.Rmd
Modified: analysis/Readdistagainstfeatures.Rmd
Modified: analysis/overlapapaqtlsandeqtls.Rmd
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Modified: code/bam2bw.sh
Modified: code/bed2saf.py
Modified: code/cluster.json
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Modified: code/config.yaml
Modified: code/environment.yaml
Modified: code/makePheno.py
Modified: code/mergeAllBam.sh
Modified: code/mergeByFracBam.sh
Modified: code/mergePeaks.sh
Modified: code/peakFC.sh
Modified: code/snakemake.batch
Modified: code/snakemakePAS.batch
Modified: code/snakemakefiltPAS.batch
Modified: code/submit-snakemake.sh
Modified: code/submit-snakemakePAS.sh
Modified: code/submit-snakemakefiltPAS.sh
Deleted: code/test.txt
Modified: data/MetaDataSequencing.txt
Modified: docs/figure/signalsiteanalysis.Rmd/figure1bMain-1.pdf
Deleted: reads_graphs.Rmd
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Rmd | 3c5e041 | brimittleman | 2019-04-29 | add write out for qtls |
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Rmd | b18b96c | brimittleman | 2019-04-29 | fix distance |
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Rmd | be90ded | brimittleman | 2019-04-21 | fix to 5perc phenp |
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Rmd | 017f5c0 | brimittleman | 2019-04-18 | add map apa qtl pipeline |
library(tidyverse)
── Attaching packages ────────────────────────────────────────────────────────────────────────────────────── tidyverse 1.2.1 ──
✔ ggplot2 3.1.1 ✔ purrr 0.3.2
✔ tibble 2.1.1 ✔ dplyr 0.8.0.1
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── Conflicts ───────────────────────────────────────────────────────────────────────────────────────── tidyverse_conflicts() ──
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library(reshape2)
Attaching package: 'reshape2'
The following object is masked from 'package:tidyr':
smiths
library(workflowr)
This is workflowr version 1.4.0
Run ?workflowr for help getting started
library(cowplot)
Attaching package: 'cowplot'
The following object is masked from 'package:ggplot2':
ggsave
In this analysis I will call apaQTls in both fractions. I will start with the phenotype files and normalized the counts using the leafcutter package in order to run the fastq QTL mapper.
It is best to run this analysis in the data/phenotype_5perc directory. I have copied the leafcutter prepare_phenotype_table.py to the code directroy to use here.
#!/bin/bash
#python2
gzip APApeak_Phenotype_GeneLocAnno.Total.5perc.fc
gzip APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc
python ../../code/prepare_phenotype_table.py APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz
python ../../code/prepare_phenotype_table.py APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz
This will output bash scripts to run.
#three-prime-env
sh APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz_prepare.sh
sh APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz_prepare.sh
Subset the PCs to use the first 2 in the qtl calling:
#three-prime-env
head -n 3 APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz.PCs > APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz.2PCs
head -n 3 APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz.PCs > APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz.2PCs
Next I will need to make a sample list. From the code directory:
python makeSampleList.py
remove 19092
Prepare directroy
mkdir ../data/apaQTLNominal
mkdir ../data/apaQTLPermuted
Run the code to call QTLs within 1mb of each PAS peak. I run both a nominal pass and a permuted pas. The permulted pas chosses the best snp for each peak gene pair.
sbatch apaQTL_Nominal.sh
sbatch apaQTL_permuted.sh
Concatinate all of the results in the permuted set. I do this so I can account for multiple testing with the benjamini hochberg test.
Concatinate results in permuted directory:
cat APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz.qqnorm_chr* > APApeak_Phenotype_GeneLocAnno.Total_permRes.txt
cat APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz.qqnorm_chr* > APApeak_Phenotype_GeneLocAnno.Nuclear_permRes.txt
Run correction script
Rscript apaQTLCorrectPvalMakeQQ.R
totRes=read.table("../data/apaQTLPermuted/APApeak_Phenotype_GeneLocAnno.Total_permResBH.txt", stringsAsFactors = F, header = T) %>% separate(pid, into=c("Chr", "Start", "End", "PeakID"), sep=":") %>% separate(PeakID, into=c("Gene", "Loc", "Strand","Peak"), sep="_")
Total Apa QTLs
TotQTLs= totRes %>% filter(-log10(bh)>=1)
nrow(TotQTLs)
[1] 377
apaQTL genes:
TotQTLs_gene=TotQTLs %>% group_by(Gene) %>% summarise(nQTL=n())
summary(TotQTLs_gene$nQTL)
Min. 1st Qu. Median Mean 3rd Qu. Max.
1.000 1.000 1.000 1.216 1.000 3.000
hist(TotQTLs_gene$nQTL)
Location distribution for peaks:
TotQTLs_loc= TotQTLs %>% group_by(Loc) %>% summarise(nLoc=n()) %>% mutate(PropLoc=nLoc/nrow(TotQTLs))
totQTLloc=ggplot(TotQTLs_loc, aes(x=Loc, y=PropLoc, fill=Loc)) + geom_bar(stat = "Identity") + labs(x="Location of Significant Peak", y="Proportion of QTLs", title="Total QTL peak distribution")+ theme(axis.text.x = element_text(angle = 90, hjust = 1))
nucRes=read.table("../data/apaQTLPermuted/APApeak_Phenotype_GeneLocAnno.Nuclear_permResBH.txt", stringsAsFactors = F, header = T) %>% separate(pid, into=c("Chr", "Start", "End", "PeakID"), sep=":") %>% separate(PeakID, into=c("Gene", "Loc", "Strand","Peak"), sep="_")
Nuclear Apa QTLs
NucQTLs= nucRes %>% filter(-log10(bh)>=1)
nrow(NucQTLs)
[1] 564
apaQTL genes:
NucQTLs_gene= NucQTLs %>% group_by(Gene) %>% summarise(nQTL=n())
summary(NucQTLs_gene$nQTL)
Min. 1st Qu. Median Mean 3rd Qu. Max.
1.000 1.000 1.000 1.253 1.000 4.000
hist(NucQTLs_gene$nQTL)
Location distribution for peaks:
NucQTLs_loc= NucQTLs %>% group_by(Loc) %>% summarise(nLoc=n()) %>% mutate(PropLoc=nLoc/nrow(NucQTLs))
nucQTLloc=ggplot(NucQTLs_loc, aes(x=Loc, y=PropLoc, fill=Loc)) + geom_bar(stat = "Identity") + labs(x="Location of Significant Peak", y="Proportion of QTLs", title="Nuclear QTL peak distribution")+theme(axis.text.x = element_text(angle = 90, hjust = 1))
plot_grid(totQTLloc, nucQTLloc)
write.table(TotQTLs, file="../data/apaQTLs/Total_apaQTLs_5fdr.txt", col.names = T, row.names = F, quote=F)
write.table(NucQTLs, file="../data/apaQTLs/Nuclear_apaQTLs_5fdr.txt", col.names = T, row.names = F, quote=F)
sessionInfo()
R version 3.5.1 (2018-07-02)
Platform: x86_64-pc-linux-gnu (64-bit)
Running under: Scientific Linux 7.4 (Nitrogen)
Matrix products: default
BLAS/LAPACK: /software/openblas-0.2.19-el7-x86_64/lib/libopenblas_haswellp-r0.2.19.so
locale:
[1] LC_CTYPE=en_US.UTF-8 LC_NUMERIC=C
[3] LC_TIME=en_US.UTF-8 LC_COLLATE=en_US.UTF-8
[5] LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8
[7] LC_PAPER=en_US.UTF-8 LC_NAME=C
[9] LC_ADDRESS=C LC_TELEPHONE=C
[11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C
attached base packages:
[1] stats graphics grDevices utils datasets methods base
other attached packages:
[1] cowplot_0.9.4 workflowr_1.4.0 reshape2_1.4.3 forcats_0.3.0
[5] stringr_1.3.1 dplyr_0.8.0.1 purrr_0.3.2 readr_1.3.1
[9] tidyr_0.8.3 tibble_2.1.1 ggplot2_3.1.1 tidyverse_1.2.1
loaded via a namespace (and not attached):
[1] Rcpp_1.0.0 cellranger_1.1.0 plyr_1.8.4 compiler_3.5.1
[5] pillar_1.3.1 git2r_0.25.2 highr_0.7 tools_3.5.1
[9] digest_0.6.18 lubridate_1.7.4 jsonlite_1.6 evaluate_0.12
[13] nlme_3.1-137 gtable_0.2.0 lattice_0.20-38 pkgconfig_2.0.2
[17] rlang_0.4.0 cli_1.1.0 rstudioapi_0.10 yaml_2.2.0
[21] haven_1.1.2 withr_2.1.2 xml2_1.2.0 httr_1.3.1
[25] knitr_1.20 hms_0.4.2 generics_0.0.2 fs_1.3.1
[29] rprojroot_1.3-2 grid_3.5.1 tidyselect_0.2.5 glue_1.3.0
[33] R6_2.3.0 readxl_1.1.0 rmarkdown_1.10 modelr_0.1.2
[37] magrittr_1.5 whisker_0.3-2 backports_1.1.2 scales_1.0.0
[41] htmltools_0.3.6 rvest_0.3.2 assertthat_0.2.0 colorspace_1.3-2
[45] labeling_0.3 stringi_1.2.4 lazyeval_0.2.1 munsell_0.5.0
[49] broom_0.5.1 crayon_1.3.4